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SPIM MOUSE

Characterization of the cellular mechanics of lineage segregation during mouse blastocyst morphogenesis by SPIM-based 4D-imaging and micromanipulation

Coordinatore	EUROPEAN MOLECULAR BIOLOGY LABORATORY Organization address address: Meyerhofstrasse 1 city: HEIDELBERG postcode: 69117 contact info Titolo: Ms. Nome: Sonja Cognome: Noss Email: send email Telefono: +49 6221 387 8771
Nazionalità Coordinatore	Germany [DE]
Totale costo	161˙968 €
EC contributo	161˙968 €
Programma	FP7-PEOPLE Specific programme "People" implementing the Seventh Framework Programme of the European Community for research, technological development and demonstration activities (2007 to 2013)
Code Call	FP7-PEOPLE-2012-IIF
Funding Scheme	MC-IIF
Anno di inizio	2014
Periodo (anno-mese-giorno)	2014-06-01 - 2016-05-31

Partecipanti

#	participant	country	role	EC contrib. [€]
1	EUROPEAN MOLECULAR BIOLOGY LABORATORY Organization address address: Meyerhofstrasse 1 city: HEIDELBERG postcode: 69117 contact info Titolo: Ms. Nome: Sonja Cognome: Noss Email: send email Telefono: +49 6221 387 8771	DE (HEIDELBERG)	coordinator	161˙968.80

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outer cell movement reconstruction axis embryo fluorescent division resolution mouse dynamics plane basis along first model sorting te inner cellular mechanistic imaging digital molecular live segregation lineage icm mechanical blastocyst

Obiettivo del progetto (Objective)

'In mammalian development, the first cell lineages are established in the blastocyst, in which the inner cell mass (ICM) and the trophectoderm (TE) occupy distinct compartment along the embryonic inner-outer axis. The inner and outer cell layers in the embryo are generated during the transition from the 8-cell to 32-cell stage in principle by two dynamic processes, cell division and cell sorting. However, the mechanism by which the spindle orientation and cellular movement are regulated in the early mouse embryo largely remains elusive. This project aims at understanding the mechanical basis of the cell lineage segregation by high-resolution fluorescent live imaging and digital reconstruction of the blastocyst patterning. To minimize photo-damage and bleaching in the embryo, we will adapt selective plane illumination microscopy (SPIM) to the mouse embryo live-imaging. Specifically, we will optimize the optical design and embryo mounting and culture for live-imaging and 4D digital reconstruction. Transgenic fluorescent reporter mice visualizing the cell membrane, the nuclei, cytoskeletons, cell polarity markers and cell adhesion proteins will allow high-resolution tracking of the lineage segregation and understanding of its mechanical basis. Our image processing will extract molecular and cellular dynamics that correlate with cell division or cell sorting along the inner-outer axis, and will establish the underlying mechanistic model. The mechanistic model will allow predicting the impact of cellular physical constraints on cell division plane and movement, and will be evaluated by experimentally testing the prediction by means of micro-manipulation. This study will thus elucidate the mechanical aspect of the ICM and TE segregation for the first time. The developed imaging system and analysis will offer a wider contribution to understanding how cellular mechanical dynamics influence molecular dynamics during development.'